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Mutated Human P-Selectin Glycoprotein Ligand-1 and Viral Protein-1 of Enterovirus 71 Interactions on Au Nanoplasmonic Substrate for Specific Recognition by Surface-Enhanced Raman Spectroscopy

DOI:10.3390/coatings10040403 期刊:Coatings 出版年份:2020 更新时间:2025-09-23 15:21:01
摘要: Protein tyrosine sulfation is a common post-translational modification that stimulates intercellular or extracellular protein-protein interactions and is responsible for various important biological processes, including coagulation, inflammation, and virus infections. Recently, human P-selectin glycoprotein ligand-1 (PSGL-1) has been shown to serve as a functional receptor for enterovirus 71 (EV71). It has been proposed that the capsid viral protein VP1 of EV71 is directly involved in this specific interaction with sulfated or mutated PSGL-1. Surface-enhanced Raman spectroscopy (SERS) is used to distinguish PSGL-1 and VP1 interactions on an Au nanoporous substrate and identify specific VP1 interaction positions of tyrosine residue sites (46, 48, and 51). The three tyrosine sites in PSGL-1 were replaced by phenylalanine (F), as determined using SERS. A strong phenylalanine SERS signal was obtained in three regions of the mutated protein on the nanoporous substrate. The mutated protein positions at (51F) and (48F, 51F) produced a strong SERS peak at 1599–1666 cm?1, which could be related to a binding with the mutated protein and anti-sulfotyrosine interactions on the nanoporous substrate. A strong SERS effect of the mutated protein and VP1 interactions appeared at (48F), (51F), and (46F, 48F). In these positions, there was less interaction with VP1, as indicated by a strong phenylalanine signal from the mutated protein.
作者: Kundan Sivashanmugan,Han Lee,Jiunn-Der Liao,Chen-Chu Wang,Chen-Hsueh Lin,Yuh-Shyong Yang,Jaya Sitjar
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Investigating the interactions between sulfated or mutated human P-selectin glycoprotein ligand-1 (PSGL-1) and viral protein-1 (VP1) of enterovirus 71 (EV71) using surface-enhanced Raman spectroscopy (SERS) on an Au nanoporous substrate for specific recognition.

The study demonstrated the use of SERS to investigate the interactions between sulfated or mutated PSGL-1 and VP1 of EV71 on an Au nanoporous substrate. Specific VP1 interaction positions were identified, and the mutated protein positions at (48F), (51F), and (46F, 48F) showed less interaction with VP1. This method contributes to understanding physiological and pathological mechanisms and aids in drug development.

The study's limitations include the need for high-purity tyrosine sulfation residues and the potential instability of sulfated target proteins in real-time applications. The method may also require optimization for broader applicability.

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